Preparation of a recombinant protein in a prokaryotic host cell

ABSTRACT

The invention relates to advantageous processes for preparing heterologous proteins in prokaryotic host cells by improved codon use and/or expression of tRNAs which code for codons occurring rarely in said host cell.

[0001] The present invention relates to advantageous processes for preparing heterologous proteins in prokaryotic host cells by improved codon use and/or expression of tRNAs which code for rarely occurring codons in the said host cell. Numerous bacteria, particularly Gram-positive bacteria, for example, have already been used as host cells for the preparation of heterologous recombinant proteins, e.g. secreted proteins, in an endotoxin-free environment (references 8, 9, 19). The bacterium Staphylococcus carnosus (S. carnosus), for example, which is used in the food industry for the fermentation of meat and fish, is a suitable bacterium for this purpose. It is free from virulence factors and proteolytic activities in the supernatant and is capable of secreting large amounts of protein (10). Moreover, only small amounts of host cell-coded proteins are secreted, which makes it easier to purify the protein produced. Bacterial enzymes (7, 4, 17), for example, have already been recombinantly produced and expressed in S. carnosus. Recombinant S. carnosus strains which express antigens such as the Streptococcus protein G on their surface,are particularly promising as live vaccines (5, 12).

[0002] One crucial disadvantage of numerous bacterial systems is their use of rare codons, which is very different from the codon preference in human genes. The presence of rare codons in E. coli led to delayed and reduced expression of recombinant genes (2, 6). The problem of the present invention is therefore to overcome this disadvantage of the prior art and provide a prokaryotic expression system with improved properties.

DESCRIPTION OF THE INVENTION

[0003] The problem is solved within the scope of the claims and specification of the present invention.

[0004] The use of the singular or plural in the claims or specification is not intended to be limiting in any way and also includes the alternative form.

[0005] The invention relates to a process for preparing a heterologous recombinant protein in a prokaryotic host cell, characterised in that the codon use of the host cell for host cell genes is determined, in the nucleic acid coding for the heterologous recombinant protein in the host cell rarely occurring codons are replaced by frequent codons, said host cell is transformed with said nucleic acid coding for the recombinant protein and said recombinant nucleic acid is expressed. With a process according to the invention it is possible to achieve a significantly better expression rate of the heterologous proteins compared with the process known from the prior art. The processes according to the invention are also particularly advantageous for the expression of recombinant proteins on the surface of prokaryotes, as the covalent anchoring on the cell wall depends on intact C-termini, which are absent from the secreted truncated proteins which are not prepared by the process according to the invention.

[0006] By heterologous is meant that said protein in said prokaryotic host cell is not native, i.e. it occurs as a protein peculiar to the host cell. “Recombinant” means produced by molecular-biological methods. A heterologous recombinant protein may be any protein known to the skilled person, such as, for example, insulin, hGH, tPA, cytokines, such as e.g. interleukins (IL) such as IL-1, IL-2, IL-3, IL-4, IL-5, IL-6, IL-7, IL-8, IL-9, IL-10, IL-11, IL-12, IL-13, IL-14, IL-15, IL-16, IL-17, IL-18, interferon (IFN) alpha, IFN beta, IFN gamma, IFN omega or IFN tau, tumour necrosis factor (TNF), TNF alpha and TNF beta, TRAIL; G-CSF, GM-CSF, M-CSF, MCP-1 and VEGF. Prokaryotic host cells may be any host cells known to the skilled person, particularly Gram-positive and Gram-negative host cells. These may be, for example, Escherichia coli, Bacillus subtilis, Streptomyces, Proteus mirabilis or preferably Staphylococcus, such as e.g. Staphylococcus carnosus in particular, as available from public collections, e.g. the Deutsche Sammlung von Mikroorganismen und Zellkulturen GmbH, Braunschweig, Germany, e.g. Strain TM300 (DSM 4600, 4601 or 4602).

[0007] Within the scope of the process according to the invention, first of all the use of the codons, i.e. the coding nucleotide triplets, is analysed for said host cell for as many native proteins as possible in the basic coding gene sequence. The codon frequencies of 51 genes were analysed for the host organism Staphylococcus carnosus Strain TM300 (10) by way of example and are shown in the following Table 1: TABLE 1 Frequency In S. Amino carnosus acid Codon (%) A (Ala) GCA 49.0 GCT 32.0 GCG 12.3 GCC  6.7 C (Cys) TGT 72.7 TGC 27.3 D (Asp) GAT 79.4 GAC 20.6 E (Glu) GAA 90.4 GAG  9.6 F (Phe) TTT 53.7 TTC 46.3 G (Gly) GGT 53.9 GGA 22.6 GGC 16.4 GGG  7.1 H (His) CAT 75.8 CAC 24.2 I (Ile) ATT 61.7 ATC 27.6 ATA 10.7 K (Lys) AAA 88.1 AAG 11.9 L (Leu) TTA 57.2 TTG 18.8 CTT 12.0 CTA  4.9 P (Pro) CCA 43.5 CTG  5.6 CTC  1.5 M (Met) ATG 100 N (Asn) AAT 64.9 AAC 35.1 CCT 31.3 CCG 23.0 CCC  2.2 Q (Gln) CAA 89.4 CAG 10.6 R (Arg) CGT 54.9 AGA 20.9 CGC 12.2 CGA 10.3 AGG  0.8 CGG  0.8 S (Ser) TCA 33.9 TCT 27.7 AGT 21.0 AGC 12.2 TCC  2.5 TCG  2.7 T (Thr) ACA 52.6 ACT 32.8 ACG 10.5 ACC  4.1 V (Val) GTT 36.7 GTA 36.7 GTG 13.6 GTC 12.9 W (Trp) TGG 100 Y (Tyr) TAT 76.4 TAC 23.6 * (Stop) TAA 68.6 TAG 19.6 TGA 11.8

[0008] It was found that coding sequences of Staphylococci for example have a very low G+C content of about 30% and the A+T-rich codons are preferred. Therefore according to the invention the production of recombinant proteins, for example hGH, is increased in two ways: (i) exchanging rare codons in the coding gene sequence for frequent ones (cf. also Example 1) and/or (ii) expressing rare tRNAs (tRNA=transfer RNA; cf. also Example 2).

[0009] The invention therefore also relates to processes for preparing a heterologous recombinant protein, wherein for S. carnosus, as shown in Table 1, or in similar manner for every other host cell according to the invention, either some or all of the rarely occurring codons are replaced by frequent ones, for example according to the analysis in Table 1 the Glu codon GAG is replaced by GAA or the Leu-codons CTC, CTG and CTA are replaced by TTA, TTG or CTT.

[0010] The invention therefore further relates to a process for preparing a heterologous recombinant protein in a prokaryotic host cell, characterised in that the codon use of the host cell for host cell genes is determined, said host cell with the nucleic acid which codes tRNA or tRNAs specific for rarely occurring codons is transformed with said nucleic acid coding for the recombinant protein, and said recombinant nucleic acid is expressed (cf. also Example 2). The skilled person can determine the rare codons of the host cell by analysing the genes or the cDNAs (or by reverse transcription of the mRNA). This has been done, for example, for the host cell S. carnosus Strain TM300 (10) in Table 1. The invention includes the introduction of tRNAs or nucleic acid coding therefore, for one to all the rare tRNAs in the host cell. Because the host cell is equipped with tRNAs which are specific for rare codons, the heterologous recombinant protein according to the invention is expressed in larger amounts than is the case in known processes from the prior art. This surprisingly advantageous property of the process according to the invention is also shown in Example 2. This may occur either on its own or in conjunction with the substitution of frequent codons for codons which are rare for the host cell in the nucleic acid coding for the heterologous protein.

[0011] Therefore the invention includes a preferred process according to the invention which is characterised in that, in the nucleic acid coding for the heterologous recombinant protein in the host cell, rarely occurring codons are replaced by frequent codons and said host cell is transformed with tRNA or tRNAs coding for rarely occurring codons and with said nucleic acid coding for the recombinant protein.

[0012] The invention includes a preferred process according to the invention which is characterised in that codons which are used in the host cell with an average frequency of less than 15% are replaced by codons with an average frequency of at least 15%;

[0013] preferably characterised in that codons which are used in the host cell with an average frequency of 7 to 12% are replaced by codons with an average frequency of more than 12%; most preferably characterised in that codons which are used in the host cell with an average frequency of up to 7 or 10% are replaced by codons with an average frequency of more than 7% or more than 10%. Another preferred embodiment is a preferred process according to the invention which is characterised in that the codon or codons which occur least often in said host cell is replaced by the codon or codons which occur most frequently in said host cell. One exception may be if said codons are absolutely essential for the expression.

[0014] The invention further includes a preferred process according to the invention which is characterised in that in the coding nucleic acid codons which are used in the host cell with an average frequency of less than 10% are replaced by codons with an average frequency of at least 10%.

[0015] The invention further includes a preferred process according to the invention which is characterised in that the host cell is Escherichia coli, as available from public collections, e.g. the Deutsche Sammlung von Mikroorganismen und Zellkulturen GmbH, Braunschweig, Germany, e.g. E. coli Strain K12 JM107 (DSM 3950).

[0016] The invention further includes a preferred process according to the invention which is characterised in that the host cell is a host cell selected from the genus Staphylococcus.

[0017] The invention further includes a preferred process according to the invention which is characterised in that the host cell is Staphylococcus carnosus (cf. also Examples 1 and 2).

[0018] In a preferred process according to the invention the recombinant protein is an antibody protein. By antibody protein is also meant a fragment, e.g. a Fab fragment (in English “Fragment antigen-binding=Fab”), a F(ab′)₂ fragment, an Fv fragment (in English: “fragment variable”=fragment of the variable part) or a single-chain Fv (scFv)), minibodies, dia-, tria- and tetrabodies.

[0019] In a preferred process according to the invention the recombinant protein is insulin.

[0020] In a preferred process according to the invention the recombinant protein is tissue plasminogen activator (tPa).

[0021] In a preferred process according to the invention the recombinant protein is a human protein.

[0022] In a preferred process according to the invention the recombinant protein is growth hormone.

[0023] In a particularly preferred process according to the invention the recombinant protein is human growth hormone (hGH, cf. Examples 1 and 2).

[0024] Another preferred process according to the invention is characterised in that G- or C-rich codons are replaced by codons containing A or T. This means that codons which contain more G or C are replaced by codons which now contain, for example, an A or a T instead of a G or C; it does not mean that the codons must now contain exclusively G or C (cf. the most preferred embodiments hereinafter).

[0025] In the process according to the invention all the rare codons found may be replaced by frequent ones (cf. e.g. Table 1) and not only those specified in the preferred embodiments given hereinafter.

[0026] Another particularly preferred process according to the invention is characterised in that the codon GCC is replaced by GCA.

[0027] Another particularly preferred process according to the invention is characterised in that the codon TGC is replaced by TGT.

[0028] Another particularly preferred process according to the invention is characterised in that the codon GAC is replaced by GAT.

[0029] Another particularly preferred process according to the invention is characterised in that the codon GAG is replaced by GAA.

[0030] Another particularly preferred process according to the invention is characterised in that the codon TTC is replaced by TTT.

[0031] Another particularly preferred process according to the invention is characterised in that the codon GGG is replaced by GGT.

[0032] Another particularly preferred process according to the invention is characterised in that the codon CAC is replaced by CAT.

[0033] Another particularly preferred process according to the invention is characterised in that the codon ATA is replaced by ATT.

[0034] Another particularly preferred process according to the invention is characterised in that the codon AAG is replaced by AAA.

[0035] Another particularly preferred process according to the invention is characterised in that the codon CTC is replaced by TTA.

[0036] Another particularly preferred process according to the invention is characterised in that the codon AAC is replaced by AAT.

[0037] Another particularly preferred process according to the invention is characterised in that the codon CCC is replaced by CCA.

[0038] Another particularly preferred process according to the invention is characterised in that the codon CAG is replaced by CAA.

[0039] Another particularly preferred process according to the invention is characterised in that the codon CGG is replaced by CGT.

[0040] Another particularly preferred process according to the invention is characterised in that the codon TCG is replaced by TCA.

[0041] Another particularly preferred process according to the invention is characterised in that the codon ACC is replaced by ACA.

[0042] Another particularly preferred process according to the invention is characterised in that the codon GTC is replaced by GTT.

[0043] Another particularly preferred process according to the invention is characterised in that the codon TAC is replaced by TAT.

[0044] Another particularly preferred process according to the invention is characterised in that the codon TGA is replaced by TAA.

[0045] Yet another preferred process according to the invention is characterised in that the host cell is transformed with the nucleic acid coding for AGG-tRNA or AGA-tRNA and with said nucleic acid coding for the recombinant protein.

[0046] The invention also particularly includes a nucleic acid molecule coding for a recombinant heterologous protein, characterised in that at least one codon rarely occurring in the host cell has been replaced by a codon which occurs frequently in the host cell. By way of example the codons for the host cell S. carnosus were analysed in Table 1. The invention includes nucleic acid molecules wherein for S. carnosus or similarly for every other host cell according to the invention either some or all of the rarely occurring codons are replaced by frequent ones, for example the Glu codon GAG is replaced by GAA or the Leu codons CTC, CTG and CTA are replaced by TTA, TTG or CTT.

[0047] The invention includes a nucleic acid molecule coding for a recombinant heterologous protein, characterised in that codons which are used in the host cell with an average frequency of less than 15% are replaced by codons with an average frequency of at least 15%; preferably characterised in that codons which are used in the host cell with an average frequency of 7 to 12% are replaced by codons with an average frequency of more than 12%; most preferably characterised in that codons which are used in the host cell with an average frequency of up to 7 or 10% are replaced by codons with an average frequency of more than 7% or more than 10%. Another preferred embodiment is a nucleic acid molecule coding for a recombinant heterologous protein, characterised in that the codon or codons which occur least often in said host cell is or are replaced by the codon or codons occurring most frequently in said host cell. One exception may be if said codons are absolutely necessary for the expression.

[0048] The invention therefore relates in a preferred embodiment to a nucleic acid molecule, characterised in that codons which are used in the host cell with an average frequency of less than 10% are replaced by codons with an average frequency of at least 10%.

[0049] The invention further relates to a nucleic acid molecule according to the invention, characterised in that it codes for the human growth hormone hGH.

[0050] The invention relates to a nucleic acid molecule, characterised in that it comprises a nucleotide sequence from the following group: the following sequence NNAGATCTAAAGGAGGTAATTCATATGAAAGAAACAAAACATCAACACACATTTTCTATCCGTAAGTCGGCTTATGGTGCCGCGTC GGTTATGGTCGCATCATGTATATTTGTCATCGGTGGGGGCGTGGCAGAGGCAAATGATTCGACAACACAAACAACGACACCACTAG AAGTCGCTCAAACGTCGCAGCAAGAAACACATACACATCAAACACCTGTTACATCATTACATACTGCAACACCTGAACATGTTGAT GACTCTAAAGAAGCAACACCTTTACCTGAAAAAGCAGAGTCACCAAAAACCGAAGTGACAGTTCAACCTTCATCGCATACACAGGA AGTACCTGCGTTACATAAAAAAACACAGCAACAACCGGCGTATAAGGATAAAACGGTACCAGAGTCAACGATAGCATCAAAGTCGG TTGAATCAAATAAAGCAACAGAAAATGAGATGTCACCTGTTGAACATCATGCTTCAAATGTGGAAAAACGTGAAGATAGATTGGAG ACTAATGAGACAACACCGCCATCAGTGGACCGTGAATTTAGCCATAAAATCATCAATAATACGCACGTAAATCCAAAAACGGATGG ACAAACAAACGTTAATGTTGATACGAAAACGATAGACACCGTTTCACCGAAAGATGACAGAATAGATACGGCGCAACCGAAACAAG TCGACGTTCCTAAAGAAAATACAACGGCACAAAATAAATTTACATCACAAGCGAGCGACAAAAAACCAACAGTAAAAGATGCATCA GGTGGTGATGATGATGATAAATTTCCAACAATTCCCTTAAGTCGATTGTTCGATAACGCTATGTTACGTGCACATAGATTACACCA GCTAGCATTCGATACTTATCAAGAATTTGAGGAAGCTTACATCCCAAAAGAACAAAAGTATAGCTTTTTACAAAATCCGCAAACAT CATTATGTTTCTCTGAATCAATTCCAACACCTAGTAACCGTGAGGAAACTCAGCAAAAATCAAATTTAGAACTTTTACGTATTAGC TTGTTACTTATACAATCTTGGTTAGAACCAGTTCAATTTTTACGTTCAGTATTCGCAAATAGTTTAGTCTATGGTGCCTCAGACTC TAACGTATACGATTTATTGAAAGACTTAGAAGAAGGAATTCAAACATTAATGGGTCGTTTGGAAGATGGTTCACCAAGAACTGGCC AAATTTTTAAACAAACATATAGCAAATTCGATACTAATTCACATAACGATGACGCATTACTTAAAAATTACGGTTTATTGTATTGT TTTCGTAAAGATATGGATAAAGTTGAAACATTCTTACGCATAGTACAATGCCGTTCTGTTGAAGGATCATGTGGTTTTTAATGATA ACTGCAG

[0051] (SEQ:ID-NO.1) or a partial sequence thereof, a nucleic acid which can hybridise with said sequence under stringent conditions, an allelic variant or a functional variant of said sequence or a variant of the nucleic acid on the basis of the degenerative code. N within the scope of the invention denotes any nucleotide known to the skilled person.

[0052] The invention further relates to a nucleic acid molecule coded by the nucleotide sequence of SEQ:ID-NO.1 NNAGATCTAAAGGAGGTAATTCATATGAAAGAAACAAAACATCAACACACATTTTCTATCCGTAAGTCGGCTTATGGTGCCGCGTC GGTTATGGTCGCATCATGTATATTTGTCATCGGTGGGGGCGTGGCAGAGGCAAATGATTCGACAACACAAACAACGACACCACTAG AAGTCGCTCAAACGTCGCAGCAAGAAACACATACACATCAAACACCTGTTACATCATTACATACTGCAACACCTGAACATGTTGAT GACTCTAAAGAAGCAACACCTTTACCTGAAAAAGCAGAGTCACCAAAAACCGAAGTGACAGTTCAACCTTCATCGCATACACAGGA AGTACCTGCGTTACATAAAAAAACACAGCAACAACCGGCGTATAAGGATAAAACGGTACCAGAGTCAACGATAGCATCAAAGTCGG TTGAATCAAATAAAGCAACAGAAAATGAGATGTCACCTGTTGAACATCATGCTTCAAATGTGGAAAAACGTGAAGATAGATTGGAG ACTAATGAGACAACACCGCCATCAGTGGACCGTGAATTTAGCCATAAAATCATCAATAATACGCACGTAAATCCAAAAACGGATGG ACAAACAAACGTTAATGTTGATACGAAAACGATAGACACCGTTTCACCGAAAGATGACAGAATAGATACGGCGCAACCGAAACAAG TCGACGTTCCTAAAGAAAATACAACGGCACAAAATAAATTTACATCACAAGCGAGCGACAAAAAACCAACAGTAAAAGATGCATCA GGTGGTGATGATGATGATAAATTTCCAACAATTCCCTTAAGTCGATTGTTCGATAACGCTATGTTACGTGCACATAGATTACACCA GCTAGCATTCGATACTTATCAAGAATTTGAGGAAGCTTACATCCCAAAAGAACAAAAGTATAGCTTTTTACAAAATCCGCAAACAT CATTATGTTTCTCTGAATCAATTCCAACACCTAGTAACCGTGAGGAAACTCAGCAAAAATCAAATTTAGAACTTTTACGTATTAGC TTGTTACTTATACAATCTTGGTTAGAACCAGTTCAATTTTTACGTTCAGTATTCGCAAATAGTTTAGTCTATGGTGCTTCAGACTC TAACGTATACGATTTATTGAAAGACTTAGAAGAAGGAATTCAAACATTAATGGGTCGTTTGGAAGATGGTTCACCAAGAACTGGCC AAATTTTTAAACAAACATATAGCAAATTCGATACTAATTCACATAACGATGACGCATTACTTAAAAATTACGGTTTATTGTATTGT TTTCGTAAAGATATGGATAAAGTTGAAACATTCTTACGCATAGTACAATGCCGTTCTGTTGAAGGATCATGTGGTTTTTAATGATA ACTGCAG

[0053] The abovementioned nucleic acid molecule according to the invention codes for hGH with the amino acid sequence of SEQ:ID-NO.2 MKETKHQHTFSIRKSAYGAASVMVASCIFVIGGGVAEANDSTTQTTTPLEVAQTSQQETHTHQTPVTSLHTATPEHVDDSKEATPL PEKAESPKTEVTVQPSSHTQEVPALHKKTQQQPAYKDKTVPESTIASKSVESNKATENEMSPVEHHASNVEKREDRLETNETTPPS VDREFSHKIINNTHVNPKTDGQTNVNVDTKTIDTVSPKDDRIDTAQPKQVDVPKENTTAQNKFTSQASDKKPTVKDASGGDDDDKF PTIPLSRLFDNAMLRAHRLHQLAFDTYQEFEEAYIPKEQKYSFLQNPQTSLCFSESIPTPSNREETQQKSNLELLRISLLLIQSWL EPVQFLRSVFANSLVYGASDSNVYDLLKDLEEGIQTLMGRLEDGSPRTGQIFKQTYSKFDTNSHNDDALLKNYGLLYCFRKDMDKV ETFLRIVQCRSVEGSCGF

[0054] according to the invention.

[0055] The invention relates to a vector containing a nucleic acid molecule according to the invention.

[0056] Another important embodiment of the invention is a host cell containing a nucleic acid molecule according to the invention or a vector according to the invention.

[0057] Another important embodiment of the invention is a host cell containing one or more tRNA molecules which codes for codons occurring rarely in this host cell.

[0058] A host cell of the genus Staphylococcus is preferred, while Staphylococcus carnosus, e.g. Strain TM300 (DSM 4600, 4601 or 4602) is most preferred.

[0059] The following Examples are intended to make the invention easier to understand and should in no way be regarded as limiting the scope of the invention.

EXAMPLE 1 Construction of a Synthetic hgH Gene with S. carnosus-specific Condon Use

[0060] As an example of a protein, human growth hormone (hGH) was expressed in S. carnosus Strain TM300.

[0061] Comparison of the codon use of the mature hGH with that shown in S. carnosus showed that 51 of the codons of the mature hGH, which represent 27% of the total number of codons, make up only 7% or less of the S. carnosus codon frequency (Tab. 2). An enterokinase cutting site was introduced at the 5′ end of the DNA sequence of the mature hGH and the hGH was synthesised with S. carnosus-specific codon use. The codons in the synthetic gene were used in about the same frequency as in the S. carnosus gene. Codons which were used by S. carnosus in a frequency of less than 10% were not used, apart from those which were needed to introduce restriction cutting sites (cf. Tab. 2). TABLE 2 Number of codons in hGH cDNA and in the synthetic hGH DNA according to the invention Amino Acid Codon ¹ ² A (Ala) GCA 1 4 GCT 1 3 GCG 0 0 GCC 5 0 C (Cys) TGT 2 3 TGC 2 1 D (Asp) GAT 2 8 GAC 9 3 E (Glu) GAA 6 12 GAG 8 2 F (Phe) TTT 4 7 TTC 9 6 G (Gly) GGT 0 5 GGA 0 2 GGC 5 1 GGG 3 0 H (His) CAT 1 2 CAC 2 1 I (Ile) ATT 2 5 ATC 6 1 ATA 0 2 K (Lys) AAA 1 8 AAG 8 1 L (Leu) TTA 1 17 TTG 0 5 CTT 1 3 CTA 4 1 CTG 12 0 CTC 8 0 M (Met) ATG 3 3 N (Asn) AAT 0 5 AAC 9 4 P (Pro) CCA 2 5 CCT 0 1 CCG 1 1 CCC 5 1 Q (Gln) CAA 2 11 CAG 11 2 R (Arg) CGT 1 7 AGA 0 2 CGC 4 1 CGA 0 1 AGG 5 0 CGG 1 0 S (Ser) TCA 3 8 TCT 3 4 AGT 1 3 AGC 6 3 TCC 4 0 TCG 1 0 T (Thr) ACA 5 6 ACT 1 4 ACG 1 0 ACC 3 0 V (Val) GTT 0 3 GTA 0 3 GTG 4 0 GTC 3 1 W(Trp) TGG 1 1 Y(Tyr) TAT 3 5 TAC 5 3 * (Stop) TAA 0 2 TAG 1 0 TGA 0 1

[0062] The synthetic hGH DNA sequence was synthesised from overlapping oligonucleotides which were hybridised and ligated in vitro. The resulting DNA fragment was cloned into the E. coli plasmid pSL1190 (3), verified by sequencing and inserted in the hGH expression cassette in order to replace the hGH cDNA between the NsiI and PstI cutting sites (FIG. 1). The new expression cassette was isolated as a BglII-ClaI fragment, cloned into the compatible BamHI and NarI cutting sites of the Staphylococci-expression vector pTX15 and transformed in S. carnosus TM300 by protoplast transformation. In the expression vector obtained, the lip-hGH fusion gene was expressed under the control of the xyl promoter of pTX15. The expression was obtained, after the inactivation of XylR, the repressor of the xyl promoter, by the addition of 0.5% xylose to the nutrient medium. The in vitro cloning and sequencing were carried out by standard methods (1). The expression of the hGH gene was performed as a fusion with the lip-signal and propeptide from Staphylococcus hyicus, which contains an enterokinase cutting site which allows the release of the mature hGH with the correct N-terminus from the fusion protein (FIG. 1). The resulting expression vector pTX-LipP-hGH4 is identical to the vector pTX-LipP-hGH2 apart from the codon use of the mature hGH. The S. carnosus strains containing one of the plasmids were cultivated in a modified LB medium (1% soya bean extract, 0.5% yeast extract, 0.5% NaCl) supplemented with 0.5% xylose, to activate the xyl promoter of the expression vectors. The use of the improved hGH DNA had a profound effect on the efficiency of the production of hGH in S. carnosus. The Lip-hGH yield was improved at least twofold and the amount of shortened Lip-hGH protein was significantly reduced (FIG. 2, traces 2 and 3). The shortened Lip-hGH proteins are not the result of extracellular proteolytic activities, as the Lip-hGH protein is stable in the S. carnosus supernatant. The reduced presence of the shortened proteins in the supernatant of S. carnosus (pTX-LipP-hGH4) shows that hGH is translated faster by the optimised DNA sequence and thus gives intracellular proteases less opportunity to cut up the protein before it is secreted away through the cytoplasmic membrane.

EXAMPLE 2 Coexpression of t-RNAs Specific for Rare Codons in hGH cDNA

[0063] The arginine codon AGG is extremely rare in S. carnosus genes, as it is used in only 0.8% of the arginine codons. The corresponding tRNA genes in S. carnosus have not yet been identified. Therefore, we expressed E. coli tRNAs for the AGG codon in S. carnosus. The E. coli genes argU and argW, which code the tRNAs for the codons AGG/AGA and AGG, had been cloned with their natural promoters and terminators into the plasmids pUBS520 or pSB101 (2, 16). The fragments were isolated as SalI-SpHI (argu) and XmaI-EcoRI (argw) fragments and cloned into the corresponding restriction cutting sites of the shuttle (transfer) vector pRB572 (4). The resulting plasmids pRBargU and pRBargW were transformed in S. carnosus (pTX-LipP-hGH2), which express hGH cDNA.

[0064] The protein patterns in the supernatant of the S. carnosus strains obtained are comparable with S. carnosus (pTX-LipP-hGH4) with increased production of the Lip-hGH protein and less truncated proteins. Therefore, the expression of rare tRNAs according to the invention has advantageous properties for the preparation of human proteins in S. carnosus, for example.

[0065] Legend Relating to the Figures

[0066]FIG. 1. Expression of the Lip-hGH fusion in the plasmids pTX- LipP-hGH2 or pTX-LipP-hGH4. The gene fusion is made up of the DNA sequences coding for the signal peptide (SP) and the propeptide (PP) from Staphylococcus hyicus lipase and the hGH part of the mature protein (in black) and is transcribed by the xyl promoter (shown as a grey triangle). The hGH cDNA or the synthetic DNA sequence was inserted between the NsiI and the PstI cutting site. The 5′ end of the hGH DNA sequence was modified to code the enterokinase cutting site ‘DDDDK’, followed by the mature hGH sequence, as shown underneath the gene.

[0067]FIG. 2. Detection of the Lip-hGH fusion proteins in the S. carnosus supernatant. Equal amounts of the supernatant were separated by SDS-PAGE on Tris-glycine gels containing 15% acrylamide and then stained with Coomassie Blue. The traces 1-5 contain supernatants of S. carnosus strains containing the empty control vector pTX16 (15), a derivative of pTX15 (trace 1), the plasmids pTX-LipP-hGH4 with the improved hGH gene (trace 2), pTX-LipP-hGH2 with the hGH cDNA (trace 3), pTX-LipP-hGH2 plus pRBargU (trace 4), and pTX-LipP-hGH2 plus pRBargW (trace 5). Standard proteins and their molecular weights (kDa) are shown on the left-hand side. The supernatants were concentrated by precipitation with trichloroacetic acid. SDS page was carried out by standard methods from the prior art.

[0068]FIG. 3. Nucleotide and amino acid sequence of the hGH according to the invention (LipPhGH4, SEQ:ID-NO.3)

[0069] Relevant restriction cutting sites are underlined once, the Shine-Dalgarno sequence is underlined twice. The signal peptidase 1 and the enterokinase cleavage site in the are underlined with a broken line. Only the regions between the BglII and NdeI site and between the NsiI and the PstI site had been synthetically produced and optimised. The remainder consists of the original sequence of the signal and propeptide of the lipase from Staphylococcus hyicus.

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[0080] 10. Götz, F. 1990. Staphylococcus carnosus: a new host organism for gene cloning and protein production. J. Appl. Bacteriol. Symp. Suppl.:49S-53S.

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[0082] 12. Liljeqvist, S., F. Cano, T. N. Nguyen, M. Uhlen, A. Robert, and S. Stahl. 1999. Surface display of functional fibronectin-binding domains on Staphylococcus carnosus. FEBS Lett. 446:299-304.

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[0084] 14. Nikoleit, K., R. Rosenstein, H. M. Verheij, and F. Götz. 1995. Comparative biochemical and molecular analysis of the Staphylococcus hyicus, Staphylococcus aureus and a hybrid lipase. Eur. J. Biochem 228:732-738.

[0085] 15. Peschel, A., B. Ottenwälder, and F. Götz. 1996. Inducible production and cellular location of the epidermin biosynthetic enzyme EpiB using an improved staphylococcal expression system. FEMS Microbiol. Lett. 137:279-284.

[0086] 16. Schenk, P. M., S. Baumann, R. Mattes, and H. H. Steinbiss. 1995. Improved high level expression system for eucaryotic genes in Escherichia coli using T7 RNA polymerase and rare Arg-tRNAs.

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1 3 1 1383 DNA Homo sapiens misc_feature (1)..(2) May be any nucleotide 1 nnagatctaa aggaggtaat tcatatgaaa gaaacaaaac atcaacacac attttctatc 60 cgtaagtcgg cttatggtgc cgcgtcggtt atggtcgcat catgtatatt tgtcatcggt 120 gggggcgtgg cagaggcaaa tgattcgaca acacaaacaa cgacaccact agaagtcgct 180 caaacgtcgc agcaagaaac acatacacat caaacacctg ttacatcatt acatactgca 240 acacctgaac atgttgatga ctctaaagaa gcaacacctt tacctgaaaa agcagagtca 300 ccaaaaaccg aagtgacagt tcaaccttca tcgcatacac aggaagtacc tgcgttacat 360 aaaaaaacac agcaacaacc ggcgtataag gataaaacgg taccagagtc aacgatagca 420 tcaaagtcgg ttgaatcaaa taaagcaaca gaaaatgaga tgtcacctgt tgaacatcat 480 gcttcaaatg tggaaaaacg tgaagataga ttggagacta atgagacaac accgccatca 540 gtggaccgtg aatttagcca taaaatcatc aataatacgc acgtaaatcc aaaaacggat 600 ggacaaacaa acgttaatgt tgatacgaaa acgatagaca ccgtttcacc gaaagatgac 660 agaatagata cggcgcaacc gaaacaagtc gacgttccta aagaaaatac aacggcacaa 720 aataaattta catcacaagc gagcgacaaa aaaccaacag taaaagatgc atcaggtggt 780 gatgatgatg ataaatttcc aacaattccc ttaagtcgat tgttcgataa cgctatgtta 840 cgtgcacata gattacacca gctagcattc gatacttatc aagaatttga ggaagcttac 900 atcccaaaag aacaaaagta tagcttttta caaaatccgc aaacatcatt atgtttctct 960 gaatcaattc caacacctag taaccgtgag gaaactcagc aaaaatcaaa tttagaactt 1020 ttacgtatta gcttgttact tatacaatct tggttagaac cagttcaatt tttacgttca 1080 gtattcgcaa atagtttagt ctatggtgct tcagactcta acgtatacga tttattgaaa 1140 gacttagaag aaggaattca aacattaatg ggtcgtttgg aagatggttc accaagaact 1200 ggccaaattt ttaaacaaac atatagcaaa ttcgatacta attcacataa cgatgacgca 1260 ttacttaaaa attacggttt attgtattgt tttcgtaaag atatggataa agttgaaaca 1320 ttcttacgca tagtacaatg ccgttctgtt gaaggatcat gtggttttta atgataactg 1380 cag 1383 2 448 PRT Homo Sapiens 2 Met Lys Glu Thr Lys His Gln His Thr Phe Ser Ile Arg Lys Ser Ala 1 5 10 15 Tyr Gly Ala Ala Ser Val Met Val Ala Ser Cys Ile Phe Val Ile Gly 20 25 30 Gly Gly Val Ala Glu Ala Asn Asp Ser Thr Thr Gln Thr Thr Thr Pro 35 40 45 Leu Glu Val Ala Gln Thr Ser Gln Gln Glu Thr His Thr His Gln Thr 50 55 60 Pro Val Thr Ser Leu His Thr Ala Thr Pro Glu His Val Asp Asp Ser 65 70 75 80 Lys Glu Ala Thr Pro Leu Pro Glu Lys Ala Glu Ser Pro Lys Thr Glu 85 90 95 Val Thr Val Gln Pro Ser Ser His Thr Gln Glu Val Pro Ala Leu His 100 105 110 Lys Lys Thr Gln Gln Gln Pro Ala Tyr Lys Asp Lys Thr Val Pro Glu 115 120 125 Ser Thr Ile Ala Ser Lys Ser Val Glu Ser Asn Lys Ala Thr Glu Asn 130 135 140 Glu Met Ser Pro Val Glu His His Ala Ser Asn Val Glu Lys Arg Glu 145 150 155 160 Asp Arg Leu Glu Thr Asn Glu Thr Thr Pro Pro Ser Val Asp Arg Glu 165 170 175 Phe Ser His Lys Ile Ile Asn Asn Thr His Val Asn Pro Lys Thr Asp 180 185 190 Gly Gln Thr Asn Val Asn Val Asp Thr Lys Thr Ile Asp Thr Val Ser 195 200 205 Pro Lys Asp Asp Arg Ile Asp Thr Ala Gln Pro Lys Gln Val Asp Val 210 215 220 Pro Lys Glu Asn Thr Thr Ala Gln Asn Lys Phe Thr Ser Gln Ala Ser 225 230 235 240 Asp Lys Lys Pro Thr Val Lys Asp Ala Ser Gly Gly Asp Asp Asp Asp 245 250 255 Lys Phe Pro Thr Ile Pro Leu Ser Arg Leu Phe Asp Asn Ala Met Leu 260 265 270 Arg Ala His Arg Leu His Gln Leu Ala Phe Asp Thr Tyr Gln Glu Phe 275 280 285 Glu Glu Ala Tyr Ile Pro Lys Glu Gln Lys Tyr Ser Phe Leu Gln Asn 290 295 300 Pro Gln Thr Ser Leu Cys Phe Ser Glu Ser Ile Pro Thr Pro Ser Asn 305 310 315 320 Arg Glu Glu Thr Gln Gln Lys Ser Asn Leu Glu Leu Leu Arg Ile Ser 325 330 335 Leu Leu Leu Ile Gln Ser Trp Leu Glu Pro Val Gln Phe Leu Arg Ser 340 345 350 Val Phe Ala Asn Ser Leu Val Tyr Gly Ala Ser Asp Ser Asn Val Tyr 355 360 365 Asp Leu Leu Lys Asp Leu Glu Glu Gly Ile Gln Thr Leu Met Gly Arg 370 375 380 Leu Glu Asp Gly Ser Pro Arg Thr Gly Gln Ile Phe Lys Gln Thr Tyr 385 390 395 400 Ser Lys Phe Asp Thr Asn Ser His Asn Asp Asp Ala Leu Leu Lys Asn 405 410 415 Tyr Gly Leu Leu Tyr Cys Phe Arg Lys Asp Met Asp Lys Val Glu Thr 420 425 430 Phe Leu Arg Ile Val Gln Cys Arg Ser Val Glu Gly Ser Cys Gly Phe 435 440 445 3 1383 DNA Artificial Sequence Homo sapiens DNA sequence flanked by vectorial DNA sequence 3 nnagatctaa aggaggtaat tcatatgaaa gaaacaaaac atcaacacac attttctatc 60 cgtaagtcgg cttatggtgc cgcgtcggtt atggtcgcat catgtatatt tgtcatcggt 120 gggggcgtgg cagaggcaaa tgattcgaca acacaaacaa cgacaccact agaagtcgct 180 caaacgtcgc agcaagaaac acatacacat caaacacctg ttacatcatt acatactgca 240 acacctgaac atgttgatga ctctaaagaa gcaacacctt tacctgaaaa agcagagtca 300 ccaaaaaccg aagtgacagt tcaaccttca tcgcatacac aggaagtacc tgcgttacat 360 aaaaaaacac agcaacaacc ggcgtataag gataaaacgg taccagagtc aacgatagca 420 tcaaagtcgg ttgaatcaaa taaagcaaca gaaaatgaga tgtcacctgt tgaacatcat 480 gcttcaaatg tggaaaaacg tgaagataga ttggagacta atgagacaac accgccatca 540 gtggaccgtg aatttagcca taaaatcatc aataatacgc acgtaaatcc aaaaacggat 600 ggacaaacaa acgttaatgt tgatacgaaa acgatagaca ccgtttcacc gaaagatgac 660 agaatagata cggcgcaacc gaaacaagtc gacgttccta aagaaaatac aacggcacaa 720 aataaattta catcacaagc gagcgacaaa aaaccaacag taaaagatgc atcaggtggt 780 gatgatgatg ataaatttcc aacaattccc ttaagtcgat tgttcgataa cgctatgtta 840 cgtgcacata gattacacca gctagcattc gatacttatc aagaatttga ggaagcttac 900 atcccaaaag aacaaaagta tagcttttta caaaatccgc aaacatcatt atgtttctct 960 gaatcaattc caacacctag taaccgtgag gaaactcagc aaaaatcaaa tttagaactt 1020 ttacgtatta gcttgttact tatacaatct tggttagaac cagttcaatt tttacgttca 1080 gtattcgcaa atagtttagt ctatggtgct tcagactcta acgtatacga tttattgaaa 1140 gacttagaag aaggaattca aacattaatg ggtcgtttgg aagatggttc accaagaact 1200 ggccaaattt ttaaacaaac atatagcaaa ttcgatacta attcacataa cgatgacgca 1260 ttacttaaaa attacggttt attgtattgt tttcgtaaag atatggataa agttgaaaca 1320 ttcttacgca tagtacaatg ccgttctgtt gaaggatcat gtggttttta atgataactg 1380 cag 1383 

1. Process for preparing a heterologous recombinant protein in a prokaryotic host cell, characterised in that the codon use of the host cell for host cell genes is determined, in the nucleic acid coding for the heterologous recombinant protein in the host cell rarely occurring codons are replaced by frequent codons, said host cell is transformed with said nucleic acid coding for the recombinant protein and said recombinant nucleic acid is expressed.
 2. Process for preparing a heterologous recombinant protein in a prokaryotic host cell, characterised in that the codon use of the host cell for host cell genes is determined, said host cell with the nucleic acid which codes tRNA or tRNAs specific for rarely occurring codons is transformed with said nucleic acid coding for the recombinant protein and said recombinant nucleic acid is expressed.
 3. Process according to claim 1 and 2, characterised in that in the nucleic acid coding for the heterologous recombinant protein in the host cell rarely occurring codons are replaced by frequent codons and said host cell is transformed with tRNA or tRNAs coding for rarely occurring codons and with said nucleic acid coding for the recombinant protein.
 4. Process according to one of claims 1 to 3, characterised in that in the coding nucleic acid, codons which are used in the host cell with an average frequency of less than 10% are replaced by codons with an average frequency of at least 10%.
 5. Process according to one of claims 1 to 4, characterised in that the host cell is Escherichia coli.
 6. Process according to one of claims 1 to 4, characterised in that the host cell is a host cell selected from the genus Staphylococcus.
 7. Process according to one of claims 1 to 4 and 6, characterised in that the host cell is Staphylococcus carnosus.
 8. Process according to one of claims 1 to 7, characterised in that the recombinant protein is an antibody protein.
 9. Process according to one of claims 1 to 7, characterised in that the recombinant protein is insulin.
 10. Process according to one of claims 1 to 7, characterised in that the recombinant protein is tissue plasminogen activator (tPa).
 11. Process according to one of claims 1 to 10, characterised in that the recombinant protein is a human one.
 12. Process according to one of claims 1 to 11, characterised in that the recombinant protein is growth hormone.
 13. Process according to one of claims 1 to 7 and 12, characterised in that the recombinant protein is human growth hormone (hGH).
 14. Process according to one of claims 1 to 13, characterised in that G- or C-rich codons are replaced by codons containing A or T.
 15. Process according to one of claims 1 to 14, characterised in that the codon GCC is replaced by GCA.
 16. Process according to one of claims 1 to 15, characterised in that the codon TGC is replaced by TGT.
 17. Process according to one of claims 1 to 16, characterised in that the codon GAC is replaced by GAT.
 18. Process according to one of claims 1 to 17, characterised in that the codon GAG is replaced by GAA.
 19. Process according to one of claims 1 to 18, characterised in that the codon TTC is replaced by TTT.
 20. Process according to one of claims 1 to 19, characterised in that the codon GGG is replaced by GGT.
 21. Process according to one of claims 1 to 20, characterised in that the codon CAC is replaced by CAT.
 22. Process according to one of claims 1 to 21, characterised in that the codon ATA is replaced by ATT.
 23. Process according to one of claims 1 to 22, characterised in that the codon AAG is replaced by AAA.
 24. Process according to one of claims 1 to 23, characterised in that the codon CTC is replaced by TTA.
 25. Process according to one of claims 1 to 24, characterised in that the codon AAC is replaced by AAT.
 26. Process according to one of claims 1 to 25, characterised in that the codon CCC is replaced by CCA.
 27. Process according to one of claims 1 to 26, characterised in that the codon CAG is replaced by CAA.
 28. Process according to one of claims 1 to 27, characterised in that the codon CGG is replaced by CGT.
 29. Process according to one of claims 1 to 28, characterised in that the codon TCG is replaced by TCA.
 30. Process according to one of claims 1 to 29, characterised in that the codon ACC is replaced by ACA.
 31. Process according to one of claims 1 to 30, characterised in that the codon GTC is replaced by GTT.
 32. Process according to one of claims 1 to 31, characterised in that the codon TAC is replaced by TAT.
 33. Process according to one of claims 1 to 32, characterised in that the codon TGA is replaced by TAA.
 34. Process according to one of claims 1 to 33, characterised in that the host cell is transformed with the nucleic acid coding for AGG-tRNA or AGA-tRNA and with said nucleic acid coding for the recombinant protein.
 35. Nucleic acid molecule coding for a recombinant heterologous protein, characterised in that at least one codon rarely occurring in the host cell has been replaced by a codon which occurs frequently in the host cell.
 36. Nucleic acid molecule according to claim 35, characterised in that codons which are used in the host cell with an average frequency of less than 10% are replaced by codons with an average frequency of at least 10%.
 37. Nucleic acid molecule according to one of claims 35 or 36, characterised in that it codes for human growth hormone hGH.
 38. Nucleic acid molecule, characterised in that it comprises a nucleotide sequence from the following group: the following sequence NNAGATCTAAAGGAGGTAATTCATATGAAAGAAACAAAACATCAACACACATTTTCTATCCGTAAGTCGGCTTATGGTGCCGCGTC GGTTATGGTCGCATCATGTATATTTGTCATCGGTGGGGGCGTGGCAGAGGCAAATGATTCGACAACACAAACAACGACACCACTAG AAGTCGCTCAAACGTCGCAGCAAGAAACACATACACATCAAACACCTGTTACATCATTACATACTGCAACACCTGAACATGTTGAT GACTCTAAAGAAGCAACACCTTTACCTGAAAAAGCAGAGTCACCAAAAACCGAAGTGACAGTTCAACCTTCATCGCATACACAGGA AGTACCTGCGTTACATAAAAAAACACAGCAACAACCGGCGTATAAGGATAAAACGGTACCAGAGTCAACGATAGCATCAAAGTCGG TTGAATCAAATAAAGCAACAGAAAATGAGATGTCACCTGTTGAACATCATGCTTCAAATGTGGAAAAACGTGAAGATAGATTGGAG ACTAATGAGACAACACCGCCATCAGTGGACCGTGAATTTAGCCATAAAATCATCAATAATACGCACGTAAATCCAAAAACGGATGG ACAAACAAACGTTAATGTTGATACGAAAACGATAGACACCGTTTCACCGAAAGATGACAGAATAGATACGGCGCAACCGAAACAAG TCGACGTTCCTAAAGAAAATACAACGGCACAAAATAAATTTACATCACAAGCGAGCGACAAAAAACCAACAGTAAAAGATGCATCA GGTGGTGATGATGATGATAAATTTCCAACAATTCCCTTAAGTCGATTGTTCGATAACGCTATGTTACGTGCACATAGATTACACCA GCTAGCATTCGATACTTATCAAGAATTTGAGGAAGCTTACATCCCAAAAGAACAAAAGTATAGCTTTTTACAAAATCCGCAAACAT CATTATGTTTCTCTGAATCAATTCCAACACCTAGTAACCGTGAGGAAACTCAGCAAAAATCAAATTTAGAACTTTTACGTATTAGC TTGTTACTTATACAATCTTGGTTAGAACCAGTTCAATTTTTACGTTCAGTATTCGCAAATAGTTTAGTCTATGGTGCTTCAGACTC TAACGTATACGATTTATTGAAAGACTTAGAAGAAGGAATTCAAACATTAATGGGTCGTTTGGAAGATGGTTCACCAAGAACTGGCC AAATTTTTAAACAAACATATAGCAAATTCGATACTAATTCACATAACGATGACGCATTACTTAAAAATTACGGTTTATTGTATTGT TTTCGTAAAGATATGGATAAAGTTGAAACATTCTTACGCATAGTACAATGCCGTTCTGTTGAAGGATCATGTGGTTTTTAATGATA ACTGCAG

(SEQ:ID-NO.1) or a partial sequence thereof, a nucleic acid which is capable of hybridising with said sequence under stringent conditions, an allelic variant or a functional variant of said sequence or a variant of the nucleic acid on the basis of the degenerative code.
 39. Nucleic acid molecule coded by the nucleotide sequence of SEQ:ID-NO.1 NNAGATCTAAAGGAGGTAATTCATATGAAAGAAACAAAACATCAACACACATTTTCTATCCGTAAGTCGGCTTATGGTGCCGCGTC GGTTATGGTCGCATCATGTATATTTGTCATCGGTGGGGGCGTGGCAGAGGCAAATGATTCGACAACACAAACAACGACACCACTAG AAGTCGCTCAAACGTCGCAGCAAGAAACACATACACATCAAACACCTGTTACATCATTACATACTGCAACACCTGAACATGTTGAT GACTCTAAAGAAGCAACACCTTTACCTGAAAAAGCAGAGTCACCAAAAACCGAAGTGACAGTTCAACCTTCATCGCATACACAGGA AGTACCTGCGTTACATAAAAAAACACAGCAACAACCGGCGTATAAGGATAAAACGGTACCAGAGTCAACGATAGCATCAAAGTCGG TTGAATCAAATAAAGCAACAGAAAATGAGATGTCACCTGTTGAACATCATGCTTCAAATGTGGAAAAACGTGAAGATAGATTGGAG ACTAATGAGACAACACCGCCATCAGTGGACCGTGAATTTAGCCATAAAATCATCAATAATACGCACGTAAATCCAAAAACGGATGG ACAAACAAACGTTAATGTTGATACGAAAACGATAGACACCGTTTCACCGAAAGATGACAGAATAGATACGGCGCAACCGAAACAAG TCGACGTTCCTAAAGAAAATACAACGGCACAAAATAAATTTACATCACAAGCGAGCGACAAAAAACCAACAGTAAAAGATGCATCA GGTGGTGATGATGATGATAAATTTCCAACAATTCCCTTAAGTCGATTGTTCGATAACGCTATGTTACGTGCACATAGATTACACCA GCTAGCATTCGATACTTATCAAGAATTTGAGGAAGCTTACATCCCAAAAGAACAAAAGTATAGCTTTTTACAAAATCCGCAAACAT CATTATGTTTCTCTGAATCAATTCCAACACCTAGTAACCGTGAGGAAACTCAGCAAAAATCAAATTTAGAACTTTTACGTATTAGC TTGTTACTTATACAATCTTGGTTAGAACCAGTTCAATTTTTACGTTCAGTATTCGCAAATAGTTTAGTCTATGGTGCTTCAGACTC TAACGTATACGATTTATTGAAAGACTTAGAAGAAGGAATTCAAACATTAATGGGTCGTTTGGAAGATGGTTCACCAAGAACTGGCC AAATTTTTAAACAAACATATAGCAAATTCGATACTAATTCACATAACGATGACGCATTACTTAAAAATTACGGTTTATTGTATTGT TTTCGTAAAGATATGGATAAAGTTGAAACATTCTTACGCATAGTACAATGCCGTTCTGTTGAAGGATCATGTGGTTTTTAATGATA ACTGCAG


40. Vector containing a nucleic acid molecule according to one of claims 35 to
 39. 41. Host cell containing a nucleic acid molecule according to one of claims 35 to 39 or a vector according to claim
 40. 42. Host cell containing one or more tRNA molecules which code for codons rarely occurring in this host cell.
 43. Host cell according to one of claims 41 or 42, characterised in that the host cell is a host cell selected from the genus Staphylococcus.
 44. Host cell according to one of claims 41 to 43, characterised in that the host cell is Staphylococcus carnosus. 